In vitro throughput screening of anticancer drugs using patient-derived cell lines cultured on vascularized three-dimensional stromal tissues

间质细胞 体外 细胞培养 吞吐量 材料科学 高通量筛选 癌症研究 生物医学工程 药理学 医学 化学 生物 生物化学 计算机科学 电信 无线 遗传学
作者
Yuki Takahashi,Rii Morimura,Kei Tsukamoto,Suguru Gomi,Asuka YAMADA,Miki Mizukami,Yasuyuki Naito,Shinji Irie,Satoshi Nagayama,Eiji Shinozaki,Kensei Yamaguchi,Naoya Fujita,Shiro Kitano,Ryohei Katayama,Michiya Matsusaki
出处
期刊:Acta Biomaterialia [Elsevier]
卷期号:183: 111-129 被引量:1
标识
DOI:10.1016/j.actbio.2024.05.037
摘要

The development of high-throughput anticancer drug screening methods using patient-derived cancer cell (PDC) lines that maintain their original characteristics in an in vitro three-dimensional (3D) culture system poses a significant challenge to achieving personalized cancer medicine. Because stromal tissue plays a critical role in the composition and maintenance of the cancer microenvironment, in vitro 3D-culture using reconstructed stromal tissues has attracted considerable attention. Here, a simple and unique in vitro 3D-culture method using heparin and collagen together with fibroblasts and endothelial cells to fabricate vascularized 3D-stromal tissues for in vitro culture of PDCs is reported. Whereas co-treatment with bevacizumab, a monoclonal antibody against vascular endothelial growth factor, and 5-fluorouracil significantly reduced the survival rate of 3D-cultured PDCs to 30%, separate addition of each drug did not induce comparable strong cytotoxicity, suggesting the possibility of evaluating the combined effect of anticancer drugs and angiogenesis inhibitors. Surprisingly, drug evaluation using eight PDC lines with the 3D-culture method resulted in a drug efficacy concordance rate of 75% with clinical outcomes. The model is expected to be applicable to in vitro throughput drug screening for the development of personalized cancer medicine. To replicate the tumor microenvironment in vitro, we constructed a cancer-stromal tissue model in which cancer cells are placed above and inside stromal tissue with vascular network structures derived from vascular endothelial cells in fibroblast tissue using CAViTs method. Using this method, we were able to reproduce the invasion and metastasis processes of cancer cells observed in vivo. Using patient-derived cancer cells, we assessed the possibility of evaluating the combined effect with an angiogenesis inhibitor. Further, primary culture was possible, suggesting that the model may be useful for new in vitro drug screening and personalized cancer medicine.
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